Non-Hodgkin Lymphoma



Non-Hodgkin Lymphoma

Protocol applies to non-Hodgkin lymphoma

involving any organ system except the

gastrointestinal tract.

Protocol revision date: January 2005

No AJCC/UICC staging system

Procedures

• Cytology (No Accompanying Checklist)

• Biopsy

• Resection of Lymph Node or Other Organ

Authors

Carolyn Compton, MD, PhD

Department of Pathology, McGill University, Montreal, Quebec, Canada

Jonathan Said, MD

Department of Pathology, UCLA School of Medicine, Los Angeles, California

For the Members of the Cancer Committee, College of American Pathologists

Previous contributors: Nancy L. Harris, MD; Dennis W. Ross, MD, PhD; Annik van den Abbeele, MD; Judith Ferry, MD; Claire Fung, MD; Irene Kuter, MD; Peter Mauch, MD

© 2005. College of American Pathologists. All rights reserved.

The College does not permit reproduction of any substantial portion of these protocols without its written authorization. The College hereby authorizes use of these protocols by physicians and other health care providers in reporting on surgical specimens, in teaching, and in carrying out medical research for nonprofit purposes. This authorization does not extend to reproduction or other use of any substantial portion of these protocols for commercial purposes without the written consent of the College.

The College of American Pathologists offers these protocols to assist pathologists in providing clinically useful and relevant information when reporting results of surgical specimen examinations of surgical specimens. The College regards the reporting elements in the “Surgical Pathology Cancer Case Summary (Checklist)” portion of the protocols as essential elements of the pathology report. However, the manner in which these elements are reported is at the discretion of each specific pathologist, taking into account clinician preferences, institutional policies, and individual practice.

The College developed these protocols as an educational tool to assist pathologists in the useful reporting of relevant information. It did not issue the protocols for use in litigation, reimbursement, or other contexts. Nevertheless, the College recognizes that the protocols might be used by hospitals, attorneys, payers, and others. Indeed, effective January 1, 2004, the Commission on Cancer of the American College of Surgeons mandated the use of the checklist elements of the protocols as part of its Cancer Program Standards for Approved Cancer Programs. Therefore, it becomes even more important for pathologists to familiarize themselves with the document. At the same time, the College cautions that use of the protocols other than for their intended educational purpose may involve additional considerations that are beyond the scope of this document.

Summary of Changes to Checklist(s)

Protocol revision date: January 2005

No changes have been made to the data elements of the checklist(s) since the January 2004 protocol revision.

Surgical Pathology Cancer Case Summary (Checklist)

Protocol revision date: January 2005

Applies to non-gastrointestinal, non-Hodgkin lymphoma only

No AJCC/UICC staging system

NON-HODGKIN LYMPHOMA: Biopsy, Resection

Patient name:

Surgical pathology number:

Note: Check 1 response unless otherwise indicated.

MACROSCOPIC

Specimen Type

___ Lymphadenectomy

___ Other (specify): ____________________________

___ Not specified

Tumor Site (check all that apply)

___ Lymph node(s), site not specified

___ Lymph node(s)

Specify site(s): _______________________________________

___________________________________________________

___ Other tissue(s) or organ(s)

Specify site(s): _______________________________________

___________________________________________________

___ Not specified

MICROSCOPIC

Histologic Type (WHO Classification)

___ Histologic type cannot be assessed

B-cell Lymphoma

___ B-cell lymphoma, subtype cannot be determined

___ Precursor B-lymphoblastic leukemia/lymphoma

___ Chronic lymphocytic leukemia/small lymphocytic lymphoma

___ B-cell prolymphocytic leukemia

___ Lymphoplasmacytic lymphoma

___ Splenic marginal zone lymphoma

___ Hairy cell leukemia

___ Plasma cell myeloma/ Plasmacytoma

___ Extranodal marginal zone B-cell lymphoma of mucosa-associated lymphoid tissue (MALT lymphoma)

___ Nodal marginal zone B-cell lymphoma

___ Follicular lymphoma, grade 1 (0-5 centroblasts per HPF)

___ Follicular lymphoma, grade 2 (6-15 centroblasts per HPF)

___ Follicular lymphoma, grade 3 (greater than 15 centroblasts per HPF)

___ Follicular lymphoma, cutaneous follicle center sub-type

___ Follicular lymphoma, diffuse follicle center sub-type, grade 1

(0-5 centroblasts per HPF)

___ Follicular lymphoma, diffuse follicle center cell sub-type, grade 2

(6-15 centroblasts per HPF)

___ Mantle cell lymphoma

___ Diffuse large B-cell lymphoma

___ Mediastinal (thymic) large B-cell lymphoma

___ Intravascular large B-cell lymphoma

___ Primary effusion lymphoma

___ Burkitt lymphoma/leukemia

___ Lymphomatoid granulomatosis

___ Other (specify): ____________________________

T-cell Lymphoma

___ T-cell lymphoma, subtype cannot be determined

___ Precursor T-lymphoblastic leukemia/lymphoma

___ T-cell prolymphocytic leukemia

___ T-cell large granular lymphocytic leukemia

___ Aggressive NK-cell leukemia

___ Adult T-cell leukemia/lymphoma

___ Extranodal NK/T-cell lymphoma, nasal type

___ Enteropathy-type T-cell lymphoma

___ Hepatosplenic T-cell lymphoma

___ Subcutaneous panniculitis-like T-cell lymphoma

___ Mycosis fungoides / Sézary syndrome

___ Primary cutaneous anaplastic large cell lymphoma

___ Peripheral T-cell lymphoma, unspecified

___ Angioimmunoblastic T-cell lymphoma

___ Anaplastic large cell lymphoma

___ Lymphomatoid papulosis

___ Other (specify): ____________________________

Extent of Pathologically Examined Tumor (check all that apply)

___ Involvement of a single lymph node region

Specify site: ____________________________

___ Involvement of multiple lymph node regions

Specify: _______________________________

___ Splenic involvement

___ Liver involvement

___ Bone marrow involvement

___ Other organ involvement

Specify: ________________________________

___Not specified

Phenotyping

___ Performed, see separate report

___ Performed

Specify method and results: ______________________________

__________________________________________________

___ Not performed

*Additional Pathologic Findings

*Specify: _______________________________________

*Comment(s)

Background Documentation

Protocol revision date: January 2005

I. Cytologic Material

A. Clinical Information

1. Patient identification

a. Name

b. Patient identification number

c. Age (birth date) (Note A)

d. Sex (Note B)

2. Responsible physician(s)

3. Date of procedure

4. Other clinical information

a. Relevant history (eg, duration of lymphadenopathy or other mass; previous diagnosis and treatment for lymphoma, Hodgkin lymphoma, or other malignancy; immunosuppression; AIDS; bone marrow or solid organ transplantation)

b. Relevant findings (eg, distribution of lymphadenopathy, signs and symptoms, imaging studies, serum lactate dehydrogenase [LDH] level) (Note C)

c. Clinical diagnosis

d. Clinical stage, if known

e. Specific procedure (fine-needle aspiration [FNA], tap of effusion, other)

f. Operative findings

g. Anatomic site(s) of specimen(s) (Note D)

B. Macroscopic Examination

1. Specimen

a. Unfixed/fixed (specify fixative)

b. Number of slides received, if appropriate

c. Quantity and appearance of fluid specimen, if appropriate

d. Other (eg, cytologic preparation from tissue)

e. Results of intraprocedural consultation

2. Material submitted for microscopic evaluation (eg, FNA, cytospin of fluid, other)

3. Special studies, specify (eg, flow cytometry for immunophenotyping, cytochemistry, immunohistochemistry, cytogenetic analysis)

C. Microscopic Evaluation

1. Adequacy of specimen (if unsatisfactory for evaluation, specify reason)

2. Lymphoma, if present

a. Histologic type, if possible (Note E)

b. Other characteristics (eg, necrosis)

3. Additional pathologic findings, if present

4. Results /status of special studies (specify)

5. Comments

a. Correlation with intraprocedural consultation, as appropriate

b. Correlation with other specimens, as appropriate

c. Correlation with clinical information, as appropriate

II. Biopsy

A. Clinical Information

1. Patient identification

a. Name

b. Patient identification number

c. Age (birth date) (Note A)

d. Sex (Note B)

2. Responsible physician(s)

3. Date of procedure

4. Other clinical information

a. Relevant history (eg, duration of lymphadenopathy or other mass; previous diagnosis and treatment for lymphoma, Hodgkin lymphoma, or other malignancy; immunosuppression; AIDS; bone marrow or solid organ transplantation)

b. Relevant findings (eg, distribution of lymphadenopathy, signs and symptoms, imaging studies, serum LDH level) (Note C)

c. Clinical diagnosis

d. Clinical stage, if known

e. Specific procedure (eg, lymph node biopsy, liver biopsy)

f. Operative findings

g. Anatomic site(s) of specimen(s) (Note D)

B. Macroscopic Examination

1. Specimen

a. Unfixed/fixed (specify fixative) (Note: When appropriate, fresh sterile tissue should be sent for culture, and fresh frozen tissue should be saved, if possible, for immunophenotyping and molecular genetic studies)

b. Number of pieces

c. Largest dimension of each piece

d. Results of intraoperative consultation

2. Submit nonfrozen tissue for microscopic evaluation

3. Special studies, specify (eg, flow cytometry for immunophenotyping, cytochemistry, immunohistochemistry, cytogenetic analysis) (Note F)

C. Microscopic Evaluation

1. Tumor

a. Histologic type (Note E)

b. Other characteristics (eg, necrosis)

2. Additional pathologic findings, if present

3. Results/status of special studies

4. Comments

a. Correlation with intraoperative consultation, as appropriate

b. Correlation with other specimens, as appropriate

c. Correlation with clinical information, as appropriate

III. Resection of Lymph Node or Other Organ

A. Clinical Information

1. Patient identification

a. Name

b. Patient identification number

c. Age (birth date) (Note A)

d. Sex (Note B)

2. Responsible physician(s)

3. Date of procedure

4. Other clinical information

a. Relevant history (eg, duration of lymphadenopathy or other mass; previous diagnosis and treatment for lymphoma, Hodgkin disease, or other malignancy; immunosuppression; AIDS; bone marrow or solid organ transplantation)

b. Relevant findings (eg, distribution of lymphadenopathy, signs and symptoms, imaging studies, serum LDH level) (Note C)

c. Clinical diagnosis

d. Clinical stage, if known

e. Specific procedure (eg, lymph node excision, splenectomy, other)

f. Operative findings

g. Anatomic site(s) of specimen(s) (Note D)

B. Macroscopic Examination

1. Specimen

a. Organ(s)/tissue(s) (Note D)

b. Unfixed/fixed (specify fixative) (Note: When appropriate, fresh sterile tissue should be sent for culture and fresh frozen tissue should be saved for immunophenotyping and molecular genetic studies)

c. Number of pieces

d. Dimensions

e. Orientation of specimen, if indicated by surgeon

f. Results of intraoperative consultation

2. Tumor

a. Number of lesions (Note G)

b. Location (Note G)

c. Configuration

d. Dimensions

e. Descriptive characteristics (eg, color, consistency)

f. Direct extension to other organ(s) or structure(s) (Note H)

g. Noncontiguous tumor involvement of other organ(s) or structure(s) (Note G)

3. Other lesions

4. Tissues submitted for microscopic evaluation

a. Lymphoma, representative sections

b. Other specific nodes, when marked by surgeon

c. Other lesions

d. Section(s) of tissue uninvolved by tumor

e. Other tissue(s)/organ(s)

5. Special studies, specify (eg, flow cytometry for immunophenotyping, cytochemistry, immunohistochemistry, cytogenetic analysis) (Note F)

C. Microscopic Evaluation

1. Tumor

a. Histologic type (Note E)

b. Direct extension to other organ(s) or structure(s)

2. Additional pathologic findings, if present (eg, reactive follicular hyperplasia)

3. Other tissues submitted (if distant involvement by lymphoma, specify site) (Note G)

4. Results/status of special studies (specify)

5. Comments

a. Correlation with intraoperative consultation, as appropriate

b. Correlation with other specimens, as appropriate

c. Correlation with clinical information, as appropriate

Explanatory Notes

A. Patient Age

Age is a risk factor independently associated with survival in non-Hodgkin lymphoma (NHL). Age above 60 years has been shown to be associated with decreased survival compared to age 60 or less.1-4 In some series of patients with low grade NHL, age greater than 40 has been associated with decreased survival.5 Across all grades and stages of NHL, a decreased ability of patients greater than 60 years of age to tolerate treatment may be the major effect of age.3 However, even among patients treated equivalently for low stage disease (ie, stage I and II, see below), older patients are at greater risk for relapse than younger patients.3,6-16

B. Sex

Across all grades and stages of NHL, male sex has been shown to correlate with other adverse prognostic factors such as histologic type, stage, and symptoms (see below). However, it has also been demonstrated to have independent adverse prognostic significance in patients with low grade NHL.5,14,17

C. Clinical Findings

Although not always provided to the pathologist by the physician submitting the specimen, certain specific clinical findings are known to be of prognostic value in NHL (across all stages). In particular, systemic symptoms of fever (greater than 38.5(C), unexplained weight loss (more than 10% body weight) in the 6 months before diagnosis, and drenching night sweats are used to define 2 categories for each stage of NHL: A (symptoms absent), and B (symptoms present). The presence of B symptoms is known to correlate with extent of disease (stage and tumor bulk), but symptoms also have been shown to have prognostic significance for cause-specific survival that is independent of stage.3,4,6,13,18,19

Poor patient “performance status” has also been shown by several multivariate analyses to have independent adverse prognostic significance.1,6,10,17 Performance status refers to the overall activity level of the patient ranging from fully active to completely bed-ridden, and a poor performance status is usually defined as any degree of activity less than fully active or fully ambulatory (ie, bed-ridden for varying proportions of time).1,2

Elevated serum lactate dehydrogenase (LDH) level is an adverse prognostic factor that correlates with tumor burden (stage and bulk).3 It has also been shown to have independent prognostic significance in both early and late stage NHL in many studies.8,12,16,20-25

Tumor bulk, usually defined by clinical and/or imaging studies, is a predictive factor in various settings.3 A tumor greater than 5 to 10 cm in diameter is associated with higher rates of relapse of stage I and II NHL treated with radiotherapy.13 A tumor greater than 10 cm in diameter is associated with poor outcome in patients with stage III and IV NHL treated with chemotherapy.3 Other definitions of bulky disease associated with poor outcome in stage II to IV NHL include a large mediastinal mass (greater than one-third of chest diameter), a palpable abdominal mass, and a combination of para-aortic and pelvic node involvement.3,4,7,13,16,17,23,26

D. Anatomic Sites

The anatomic sites that constitute the major structures of the lymphatic system include groups and chains of lymph nodes, the spleen, the thymus, Waldeyer’s ring (a circular band of lymphoid tissue that surrounds the oropharynx consisting of the palatine, lingual, and pharyngeal tonsils), the vermiform appendix, and the Peyer’s patches of the ileum. Minor sites of lymphoid tissue include the bone marrow, liver, skin, lung, pleura, and gonads. Involvement of extranodal sites is more common in NHL than in Hodgkin lymphoma.

E. Histologic Type

The protocol recommends the World Health Organization (WHO) Classification of Lymphoid Neoplasms, which is shown below.27,28 This classification encompasses both nodal and extranodal lymphomas and outlines the immunobiologic features of the defined entities that aid in the diagnosis. The prognostic information necessary to determine treatment of lymphoma is, in general, provided by the histologic type.

WHO Classification of Lymphoid Neoplasms

B-cell Neoplasms

Precursor B-cell neoplasms

Precursor B-lymphoblastic lymphoma/leukemia

Mature B-cell neoplasms

Chronic lymphocytic leukemia/small lymphocytic lymphoma

Variant: Mu heavy chain disease

B-cell prolymphocytic leukemia

Lymphoplasmacytic lymphoma / Waldenström macroglobulinemia

Variant: Gamma heavy chain disease

Splenic marginal zone lymphoma

Hairy cell leukemia

Variant: Hairy cell variant

Plasma cell myeloma

Solitary plasmacytoma of bone

Extraosseous plasmacytoma

Extranodal marginal zone B-cell lymphoma of mucosa-associated lymphoid tissue (MALT lymphoma )

Nodal marginal zone B-cell lymphoma

Follicular lymphoma

Grading:

Grade 1: 0 to 5 centroblasts per high power field#

Grade 2: 6 to 15 centroblasts per high power field#

Grade 3: greater than 15 centroblasts per high power field#

Grade 3a: centrocytes are still present

Grade 3b: centroblasts form solid sheets with no residual centrocytes

Reporting of pattern:

Follicular: greater than 75% follicular

Follicular and diffuse: 25% to 75% follicular

Focally follicular: less than 25% follicular

Variants:

Cutaneous follicle center lymphoma

Diffuse follicle center lymphoma

Grade 1: 0 to 5 centroblasts per high power field#

Grade 2: 6 to 15 centroblasts per high power field#

Mantle cell lymphoma

Variants: Blastoid (classic or pleomorphic), others

Diffuse large B-cell lymphoma

Mediastinal (thymic) B-cell lymphoma

Intravascular large B-cell lymphoma

Primary effusion lymphoma

Morphologic variants:

Centroblastic

Immunoblastic

T-cell/histiocyte-rich

Anaplastic

Burkitt lymphoma

Variants:

Burkitt lymphoma with plasmacytoid differentiation

Atypical Burkitt/Burkitt-like

B-cell proliferations of uncertain malignant potential

Lymphomatoid granulomatosis

Post-transplant lymphoproliferative disorder, polymorphic

# WHO guideline27 for high powered field (HPF) = high powered field of 0.159mm2 (40X objective, 18mm field of view ocular; count 10 HPF and divide by 10). If using a 10mm field of view ocular, count 8 HPF and divide by 10, or count 10 HPF and divide by 12 to get the number of centroblasts/0.159mm2 HPF. If using a 22-mm field of view ocular, count 7 HPF and divide by 10, or count 10 HPF and divide by 15 to get the number of centroblasts/0.159mm2 HPF.

T-cell Neoplasms

Precursor T-cell neoplasms

Precursor T lymphoblastic lymphoma/leukemia

Blastic NK-cell lymphoma

Mature T-cell and NK-cell neoplasms

T-cell prolymphocytic leukemia

Variants: small cell, cerebriform cell (Sézary cell-like)

T-cell granular lymphocyte leukemia

Aggressive NK-cell leukemia

Adult T-cell lymphoma/leukemia (HTLV1+)

Clinical variants:

Acute

Lymphomatous

Chronic

Smoldering

Extranodal NK/T-cell lymphoma, nasal type

Enteropathy-type T-cell lymphoma

Hepatosplenic T-cell lymphoma

Variants: gamma-delta T-cell lymphoma in other anatomic sites

(eg, skin, intestine)

Subcutaneous panniculitic-like T-cell lymphoma

Blastic NK-cell lymphoma

Mycosis fungoides (MF) and Sézary syndrome

Variants:

Pagetoid reticulosis

MF-associated follicular mucinosis

Granulomatous slack skin disease

Primary cutaneous anaplastic large cell lymphoma (C-ALCL)

Peripheral T-cell lymphoma, unspecified

Angioimmunoblastic T-cell lymphoma

Anaplastic large cell lymphoma

T-cell proliferation of uncertain malignant potential

Lymphomatoid papulosis

Immunophenotypes and Genetics26-29

Precursor B lymphoblastic leukemia/lymphoma: Slg-, cytoplasmic µ chain 30%, CD19+, CD20-/+, CD22+, CD79a+, TdT+, HLA-DR+, CD10+/-, CD34+/-,

CD13-/+, CD33-/+, IgH gene rearrangement +/-, IgL gene rearrangement -/+, TCR gene rearrangement -/+, variable cytogenetic abnormalities

B-cell chronic lymphocytic leukemia (B-CLL): Faint SIgM+, SIgD+/-, CIg-/+, panB+ (CD19+, CD20+), CD5+, CD10-, CD23+, CD43+, CD11c-/+; IgH and IgL gene rearrangements; trisomy 12-/+; 13q abnormalities-/+

Lymphoplasmacytic lymphoma: SIgM+, SIgD-/+, CIg+, PanB+, CD5-, CD10-, CD43+/-, CD25-/+; IgH and IgL gene rearrangements

Splenic marginal zone lymphoma: SIgM+, SIgD+, CD20+, CD79a+, CD5-, CD10-, CD23-, CD43-, nuclear cyclin D1-, CD103-, allelic loss at 7q21-32 (40% of cases)

Hairy cell leukemia: SIg+ (IgM, IgD, IgG, or IgA), PanB+, CD79a+, CD79b-, DBA.44+, CD5-, CD10-, CD23-, CD11c+, CD25+, FMC7+, CD103+ (mucosal lymphocyte antigen as detected by B-ly7), tartrate resistant acid phosphatase (TRAP)+; IgH and IgL gene rearrangements

Plasma cell myeloma: CIg+ (IgG, IgA, rare IgD, IgM, or IgE or light chain only), PanB-, (CD19-, CD20-, CD22-), CD79a+/-, CD45-/+, HLA-DR-/+, CD38+, CD56+/-, EMA-/+, CD43+/-; IgH and IgL gene rearrangements; deletions most commonly 13q, and occasional translocations, in particular t(11;14)(q13;q32)

Extranodal marginal zone B-cell lymphoma of MALT ( MALT lymphoma): SIg+ (IgM or IgA or IgG), SIgD-, CIg-/+, PanB+, CD5-, CD10-, CD23-, CD43-/+; IgH and IgL gene rearrangements, bcl-1 and bcl-2 germline, trisomy 3 or t(11;18)(q21;q21) may be seen

Nodal marginal zone B-cell lymphoma : SIgM+, SIgD-, CIg-/+, PanB+, CD5-, CD10-, CD23-, CD43-/+; IgH and IgL gene rearrangements, bcl-1 and bcl-2 germline

Follicular lymphoma: SIg+ (usually IgM +/- IgD, IgG, IgA), PanB+, CD10+/-, CD5-, CD23-/+, CD43-, CD11c-, CD25-; overexpression of BCL-2+ (useful to distinguish from reactive follicles); BCL6+ IgH and IgL gene rearrangements, t(14;18) with rearranged BCL-2 gene in 70-95% of cases

Mantle cell lymphoma: SIgM+, SIgD+, lambda>kappa, PanB+, CD5+, CD10-/+, CD23-, CD43+, CD11c-, CD25-; IgH and IgL gene rearrangements, t(11;14); bcl-1 gene rearrangements (CCND1/cyclinD1/PRAD1) common

Diffuse large B-cell lymphoma: SIg+/-, CIg-/+, PanB+, CD45+/-, CD5-/+, CD10-/+ (weak); IgH and IgL gene rearrangements; bcl-2 gene rearranged in 30% of cases, bcl-6/LAZ3 gene (chromosome 3q27) rearranged in 30% of cases, c-myc gene rearrangement uncommon

Mediastinal (thymic) large B-cell lymphoma: SIg-/+, PanB+, (especially CD20, CD79a), CD45+/-, CD15-, CD30-/+ (weak); IgH and IgL gene rearrangements

Burkitt lymphoma: SIgM+, PanB+, CD5-, CD10+, CD23-; IgH and IgL gene rearrangements, t(8;14) and variants t(2;8) and t(8;22); rearranged c-myc gene. EBV common (95%) in endemic cases and infrequent (15-20%) in sporadic cases, intermediate incidence (30-40%) in HIV-positive cases

Atypical Burkitt/ Burkitt-like lymphoma: SIg+/- (IgM or IgG), CIg-/+, PanB+, CD5-, CD10-/+; IgH and IgL gene rearrangements, infrequent rearrangement of c-myc gene, bcl-2 gene rearranged in 30% of cases

Precursor T-lymphoblastic lymphoma/leukemia: TdT+, CD7+, CD3+/-, variable expression of other PanT antigens, CD1a+/-, often CD4 and CD8 double positive or negative, Ig-, PanB-; variable rearrangement of TCR genes; IgH gene rearrangement -/+, most common chromosomal abnormalities involve 14q11-14 or 7q35; variable cytogenetic abnormalities reported

T-cell prolymphocytic leukemia: TdT-, PanT+, (CD2, CD3, CD5, CD7) CD25-, CD4+/CD8->CD4+/CD8+>CD4-/CD8-; TCR gene rearrangements, 75% of cases show inv 14(q11;q32)

T-cell large granular lymphocytic leukemia, T-cell type: TdT-, PanT+ (CD2, CD3+, CD5+/-, CD7-), TCR+, CD4-, CD8+, CD16+, CD56-, CD57+, CD25-; most cases show clonal rearrangements of TCR genes

T- cell large granular lymphocytic leukemia, NK-cell type: TdT-, CD2+, CD3-, TCR-, CD4-, CD8+/-, CD16+/-, CD56+/-, CD57+/-, CD25-; TCR and Ig genes are germline

Adult T-cell lymphoma/leukemia (HTLV1+): TdT-, PanT+ (CD2+, CD3+, CD5+, CD7-) CD4+, CD8-, CD25+; TCR gene rearrangements, clonally integrated HTLV1

Extranodal NK/T-cell lymphoma, nasal type: TdT-, CD2+, CD5-/+, CD7-/+, CD3-/+, may be CD4+ or CD8+, CD56+/-; usually no rearranged TCR or Ig genes; often EBV positive

Enteropathy-type T-cell lymphoma: TdT-, CD3+, CD7+, CD4-, CD8+/-, CD103+ (mucosal lymphocyte antigen, such as detection by HML-1) (see gastrointestinal lymphoma protocol)

Hepatosplenic T-cell lymphoma : CD2+, CD3+, TCR gamma-delta+, TCRab-, CD5-, CD7+, CD4-, CD8-/+, CD56+/-, CD25-; TCR- gene rearrangements, variable TCR- gene rearrangements

Mycosis fungoides/Sézary syndrome: TdT-, PanT+ (CD2+, CD3+, CD5+, CD7-/+), most cases CD4+/CD8-, CD25-/+; TCR gene rearrangements

Angioimmunoblastic T-cell lymphoma: TdT-, PanT+ (often with variable loss of some PanT antigens), usually CD4+; TCR gene rearrangements in 75%; IgH gene rearrangements in 10%, EBV often positive, but usually only in isolated neoplastic or reactive cells

Peripheral T-cell lymphomas, unspecified: TdT-, PanT variable (CD2+/-, CD3+/-, CD5+/-, CD7-/+), most cases CD4+, some cases CD8+, CD4-/CD8-, or CD4+/CD8+; TCR gene rearrangements usual

Anaplastic large cell lymphoma: TdT-, CD30+, EMA+/-, PanT-/+, CD45+/-, CD25+/-,

CD15-/+, CD68-, lysozyme-, BNH9+/-; primary cutaneous form is EMA- and cutaneous lymphocyte antigen+; TCR gene rearrangements > germline, 12-50% of adult cases show t(2;5) resulting in a fusion on NPM gene (5q35) with ALK gene (2q23)

F. Special Studies: Specimen Handling

Specimens for the diagnosis of lymphoma require special handling in order to optimize the histologic diagnosis and to prepare the tissue for performance of molecular and other special studies. The guidelines detailed below are suggested for specimen handling in cases of suspected lymphoma.

• Tissue should be received fresh. Unsectioned lymph nodes should not be immersed in fixative.

• The fresh specimen size, color and consistency should be recorded, as should the presence or absence of any visible nodularity, hemorrhage, or necrosis after serial sectioning at 2-mm intervals perpendicular to the long axis of a lymph node.

• Touch imprints may be made from the freshly cut surface, and the imprints fixed in alcohol or air dried.

• For cytogenetic studies or culture of microorganisms: submit a portion of the node sterilely in appropriate medium.

• Fixation (record fixative[s] used for individual slices of the specimen):

• B5 produces superior cytologic detail but is not suitable for DNA extraction and may impair some immunostains (eg, CD30).

• Over-fixation (ie, more than 24 hours in formalin, more than 4 hours in B5) should be avoided.

• Snap-frozen tissue is optimal for some immunostains and for DNA and RNA extractions.

• Cover tissue samples (cut to approximately 1x1x0.3 cm) in OCT.

• Immerse in dry ice/isopentane slush or liquid nitrogen.

• Store at -80(C until needed.

G. Stage

In general, the TNM classification has not been used for staging of lymphomas because the site of origin of the tumor is often unclear and there is no way to differentiate among T, N, and M. Thus, a special staging system (Ann Arbor System) is used for both Hodgkin lymphoma and NHL. The Ann Arbor classification for lymphomas has been applied to NHL by the American Joint Committee (AJCC) on Cancer and the International Union Against Cancer (UICC) (see below).30,31 For multiple myeloma, the Durie-Salmon staging system is recommended by the AJCC. Both staging systems are shown below.

Pathologic staging depends on biopsy or resection of one or more regional lymph nodes, splenectomy, wedge liver biopsy, bone marrow biopsy, and biopsy of multiple lymph nodes on both sides of the diaphragm to assess distribution of disease. Clinical staging generally involves a combination of clinical, radiologic, and surgical procedures and includes medical history, physical examination, laboratory tests (eg, complete blood examination, and blood chemistry studies), imaging studies (eg, computed tomography [CAT] scans, magnetic resonance imaging [MRI] studies, and nuclear medicine studies), biopsy to determine diagnosis, extent of disease, and histologic type of tumor (initial diagnosis is almost always made on biopsy), and often bone marrow biopsy. Most commonly, staging of NHL is clinical rather than pathologic.

There is almost universal agreement that the stage of NHL is prognostically

significant.1-3,6,8,13,17,21

AJCC/UICC Staging for Non-Hodgkin Lymphomas30,31

Stage I Involvement of a single lymph node region (I) or localized involvement of a single extralymphatic organ or site in the absence of any lymph node involvement (IE)#, ##

Stage II Involvement of 2 or more lymph node regions on the same side of the diaphragm (II), or localized involvement of a single extralymphatic organ or site in association with regional lymph node involvement with or without involvement of other lymph node regions on the same side of the diaphragm (IIE) ##,###

Stage III Involvement of lymph node regions on both sides of the diaphragm (III), which also may be accompanied by extralymphatic extension in association with adjacent lymph node involvement (IIIE) or by involvement of the spleen (IIIS) or both (IIIE+S) ##,###, ^

Stage IV Diffuse or disseminated involvement of 1 or more extralymphatic organs, with or without associated lymph node involvement; or isolated extralymphatic organ involvement in the absence of adjacent regional lymph node involvement, but in conjunction with disease in distant site(s). Any involvement of the liver or bone marrow, or nodular involvement of the lung(s). ##,###,^

# Multifocal involvement of a single extralymphatic organ is classified as stage IE and not stage IV.

## For all stages, tumor bulk greater than 10 to 15 cm is an unfavorable prognostic factor.3

### The number of lymph node regions involved may be indicated by a subscript: eg, II3. For stages II to IV, involvement of more than 2 sites is an unfavorable prognostic factor.3

^ For stages III to IV, a large mediastinal mass is an unfavorable prognostic factor.3

AJCC/UICC Staging for Plasma Cell Myeloma30,31

Stage I Hemoglobin greater than 10.0 g/dL

Serum calcium 12 mg/dL or less

Normal bone x-rays or a solitary bone lesion

IgG less than 5 g/dL

IgA less than 3 g/dL

Urine M-protein less than 4 g/24 hours

Stage III One or more of the following are included:

Hemoglobin greater than 8.5 g/dL

Serum calcium greater than 12 mg/dL

Advanced lytic bone lesions

IgG greater than 7 g/dL

IgA greater than 5 g/dL

Urine M-protein less than 12 g/24 hours

Stage II Disease fitting neither stage I nor stage III

Note: Patients are further classified as (A) serum creatinine less than 2.0 mg/dL, or (B) serum creatinine 2.0 mg/dL or greater. The median survival for stage IA disease is about 5 years, and that for stage IIIB disease is 15 months.30

H. Direct Spread into Adjacent Tissues or Organs

Direct spread of a lymphoma into adjacent tissues or organs does not influence classification of stage.

References

1. Shipp MA, Harrington DP, Anderson JR, et al. A predictive model for aggressive non-Hodgkin lymphoma. N Engl J Med. 1993;329:987-994.

2. Shipp MA. Prognostic factors in aggressive non-Hodgkin lymphoma. Blood. 1994;83:1165-1173.

3. Crump M, Gospodarowicz MK. Non-Hodgkin malignant lymphoma. In: Gospodarowicz MK, Henson DE, Hutter RVP, O’Sullivan B, Sobin LH, Wittekind C, eds. Prognostic Factors in Cancer. New York, NY: Wiley-Liss; 2001:689-703.

4. Gospodarowicz MK, Bush RS, Brown TC, et al. Prognostic factors in nodular lymphomas: a multivariate analysis based on the Princess Margaret experience. Int J Radiat Oncol Biol Phys. 1984;10:489-497.

5. Dana BW, Dahlberg S, Nathwani BN, et al. Long-term follow-up of patients with low-grade malignant lymphomas treated with doxorubicin-based chemotherapy or chemoimmunotherapy. J Clin Oncol. 1993;11:644-651.

6. Hayward RL, Leonard RC, Prescott RJ, et al. A critical analysis of prognostic factors for survival in intermediate and high grade non-Hodgkin lymphoma: Scotland and Newcastle Lymphoma Group Therapy Working Party. Br J Cancer. 1991;63:945-952.

7. Kaminski MS, Coleman CN, Colby TV, et al. Factors predicting survival in adults with stage I and II large-cell lymphoma treated with primary radiation therapy. Ann Intern Med. 1986;104:747-56.

8. Lindh J, Lenner P, Osterman B, et al. Prognostic significance of serum lactic dehydrogenase levels and fraction of S-phase cells in non-Hodgkin lymphomas. Eur J Hematol. 1993;50:258-263.

9. O’Reilly SE, Hoskins P, Klimo P, et al. MACOP-B and VACOP-B in diffuse large lymphomas and MOPP/ABV in Hodgkin disease. Ann Oncol. 1991;1:17-23.

10. Shimoyama M, Ota K, Kitutchi M, et al. Major prognostic factors of adult factors of adult patients with advanced B-cell lymphoma treated with vincristine, cyclophosphamide, prednisone and doxorubicin (VEPA) or VEPA plus methotrexate (VEPA-M). Jpn J Clin Oncol. 1988;18:113-124.

11. Soubeyran P, Eghbali H, Bonichon, et al. Localized follicular lymphomas: prognosis and survival of stage I and II in a retrospective series of 103 patients. Radiother Oncol. 1988;13:91-98.

12. Stein RS, Greer JP, Cousar JB, et al. Malignant lymphomas of follicular centre cell origin in man, VII: prognostic features in small cleaved lymphoma. Hematol Oncol. 1989;7:381-391.

13. Sutcliffe SB, Gospodarowicz MK, Bush RS, et al. Role of radiation therapy in localized non-Hodgkin lymphoma. Radiother Oncol. 1985;4:211-223.

14. Taylor RE, Allan SG, McIntyre MA, et al. Low grade stage I and II non-Hodgkin lymphoma: results of treatment and relapse pattern following therapy. Clin Radiol. 1988;39:287-290.

15. Velasquez WS, Fuller LM, Jagannath S, et al. Stages I and II diffuse large cell lymphomas: prognostic factors and long-term results with CHOP-bleo and radiotherapy. Blood. 1991;77:942-947.

16. Velasquez WS, Jagannath S, Tucker TS, et al. Risk classification as the basis for clinical staging of diffuse large-cell lymphoma derived from 10-year survival data. Blood. 1989;74:551-557.

17. Steward WP, Crowther D, McWilliam LJ, et al. Maintenance chlorambucil after CVP in the management of advanced stage, low grade histologic type non-Hodgkin lymphoma: a randomized prospective study with assessment of prognostic factors. Cancer. 1988;61:441-447.

18. Hoskins PJ, Ng V, Spinelli JJ, et al. Prognostic variables in patients with diffuse large-cell lymphoma treated with MACOP-B. J Clin Oncol. 1991;9:220-226.

19. O’Reilly SE, Hoskins P, Klimo P, et al. Long-term follow-up of pro-MACE-CytoBOM in non-Hodgkin lymphoma. Ann Oncol. 1991;1:33-35.

20. Bastion Y, Berger F, Bryon PA, et al. Follicular lymphomas: assessment of prognostic factors in 127 patients followed for 10 years. Ann Oncol. 1991;(suppl 2):123-129.

21. Cowan RA, Jones M, Harris M, et al. Prognostic factors in high and intermediate grade non-Hodgkin lymphoma. Br J Cancer. 1989;59:276-282.

22. Kwak LW, Halpern J, Olshen RA, et al. Prognostic significance of actual dose intensity in diffuse large-cell lymphoma: results of a tree-structured survival analysis. J Clin Oncol. 1990;8:963-977.

23. Prestidge BR, Horning SJ, Hoppe RT. Combined modality therapy for stage I-II large cell lymphoma. Int J Radiat Oncol Biol Phys. 1988;15:633-639.

24. Straus DJ, Wong G, Yahalom J, et al. Diffuse large cell lymphoma: prognostic factors with treatment. Leukemia. 1991;1:32-37.

25. Vitolo U, Bertini M, Brusamolina E, et al. MACOP-B treatment in diffuse large cell lymphoma: identification of prognostic groups in an Italian multicenter study. J Clin Oncol. 1992;10:219-227.

26. Jaffe ES, Harris NL, Stein H, Vardiman JW, eds. World Health Organization Classification of Tumours. Pathology and Genetics. Tumours of Haematopoietic and Lymphoid Tissues. Lyon (France): IARC Press; 2001.

27. Stein H, Delsol G, Pileri S, et al. WHO histological classification of Hodgkin lymphoma. In: Jaffe ES, Harris NL, Stein H, Vardiman JW, eds. World Health Organization Classification of Tumours. Pathology and Genetics. Tumours of Haematopoietic and Lymphoid Tissues. Lyon (France): IARC Press; 2001.

28. Harris NL, Jaffe ES, Stein H, et al. A revised European-American classification of lymphoid neoplasms: a proposal from the International Lymphoma Study Group. Blood. 1994;84:1361-1392.

29. Chan JKC, Banks PM, Cleary ML, et al. A revised European-American classification of lymphoid neoplasms: a proposal from the International Lymphoma Study Group: a summary version. Am J Clin Pathol. 1995;103:543-560.

30. Greene FL, Page DL, Fleming ID, et al, eds. AJCC Cancer Staging Manual. 6th ed. New York: Springer; 2002.

31. Sobin LH, Wittekind C, eds. UICC TNM Classification of Malignant Tumours. 6th ed. New York: Wiley-Liss; 2002.

Bibliography

Coiffier B, Gisselbrecht C, Vose JM, et al. Prognostic factors in aggressive malignant lymphomas: description and validation of a prognostic index that could identify patients requiring a more intensive therapy. J Clin Oncol. 1991;9:211-219.

Collins RD. Lymph node examination: what is an adequate work-up? Arch Pathol Lab Med. 1985;109:796-9.

Cousar JB. Surgical pathology examination of lymph nodes. Am J Clin Pathol. 1995;104:126-132.

Gordon LI, Andersen J, Colgan J, et al. Advanced non-Hodgkin lymphoma: analysis of prognostic factors by the International Index and by lactic dehydrogenase in an intergroup study. Cancer. 1995;75:865-873.

Kramer MHH, Hermans J, Parker J, et al. Clinical significance of bcl2 and p53 protein expression in diffuse large B-cell lymphoma: a population-based study. J Clin Oncol. 1996;14:2131-2138.

Liang R, Todd D, Ho FC: Aggressive non-Hodgkin lymphoma: T-cell versus B-cell. Hematol Oncol. 1996;14:1-6.

Osterman B, Cavallin-Stahl E, Hagberg H, et al. High-grade non-Hodgkin lymphoma stage I: a retrospective study of treatment, outcome, and prognostic factors in 213 patients. Acta Oncol. 1996;35:171-177.

Stauder R, Eisterer W, Thaler J, et al. CD44 variant isoforms in non-Hodgkin’s lymphoma: a new independent prognostic factor. Blood. 1995;85:2885-2889.

................
................

In order to avoid copyright disputes, this page is only a partial summary.

Google Online Preview   Download